对毛细管电泳法和亲合液相色谱法测定保健食品中免疫球蛋白G的改进

对现行的毛细管电泳法和亲合液相色谱法测定保健食品中免疫球蛋白G(IgG)的方法作了两方面的改进:①在样品的预处理方面,采用加入稀乙酸使酪蛋白沉淀析出并用离心法预以分离;②在亲合液相色谱测定方法方面,用内径较大(0.51mm)的不锈钢管道系统代替了原有的系统,使系统的反压值下降至276kPa,达到与免疫亲合色谱柱的耐压最大值300kPa相匹配。改进后的方法的线性范围在200～2000mg·L~(-1)之间。在分别加入100,300mg·L~(-1)标准IgG溶液的浓度水平上做了回收试验,测得方法的回收率和相对标准偏差(n=5)依次为112%和97%以及4.2%和3.9%。13种保健食品样品中IgG含量的亲合液相色谱法测定结果与毛细管电泳法的测定结果相一致。     

普鲁士蓝增敏压电均相免疫分析法测定免疫球蛋白G

建立了普鲁士蓝增敏的均相压电免疫分析法,用于人尿液中免疫球蛋白G(IgG)的检测.本方法以蛋白质为种子,形成蛋白质-普鲁士蓝粒子,该粒子不断“滚雪球”增大,使得压电检测信号明显放大.在pH 4.0、盐浓度0.1 mol/L,5 mmol/L FeC13,2.5 mmol/L K4Fe(CN)6(K4Fe(CN)6与蛋白浓度比≥5000),FeCl3加样速度为0.5 μL/s的优化条件下,IgG的检测范围为0～625 nmol/L;检出限为2.4 nmol/L.α1-微球蛋白,β2-微球蛋白、尿微量白蛋白均无明显干扰.本方法用于临床样本的IgG测定,并与免疫比浊法进行对比,两者结果一致,表明本方法可行.     

大孔及涂敷硅球作基质的组氨酸拟亲和色谱纯化人免疫球蛋白G

研究用分子组氨酸和配体、大孔硅球为基质的拟亲和色谱分离纯化人免疫蛋白Ｇ（ＩｇＧ），认为键合组氨酸具有半抗原体质而与ＩｇＧ发生免疫亲和作用，以色谱组份重新进样验证了色谱柱对ＩｇＧ亲和专一性，并用包敷Ｄｅｘｔｒａｎ大孔硅球作基质的拟亲和色谱纯化人血清中的ＩｇＧ，减少了色谱峰拖尾，缩短了分离时间。     

基于胶体金标记的阳极溶出伏安免疫分析用于免疫球蛋白G的测定

提出了一种基于胶体金标记的阳极溶出伏安免疫分析方法。免疫反应在聚苯乙烯微孔板中以夹心分析模式进行,通过物理吸附将兔抗人免疫球蛋白G(IgG)抗体固定于微孔板上,与相应抗原IgG发生免疫反应后,再通过夹心模式捕获相应的纳米金标记的羊抗人IgG抗体,然后再与金标羊抗人IgG抗体和金标兔抗羊二抗形成的免疫复合物反应,在微孔板上进一步引入大量的纳米金,将金溶解后,在碳糊电极上用阳极溶出伏安法(ASV)对金离子进行检测,溶出峰电流的大小间接与待分析物IgG的浓度成正比。对免疫分析的一些实验条件进行了优化。阳极溶出峰电流与IgG的对数浓度在1.1~1 143 ng/mL范围内呈良好的线性关系,检出限为1 ng/mL。将该方法应用于人血清中IgG浓度的测定,取得了满意结果。     

新型pH敏感高分子相分离荧光免疫分析法测定兔血清中IgG

通过将N-异丙基丙烯酰胺（NIP）、甲基丙烯酸丁酯（BMA）和甲基丙烯酸（MAA）共聚得到了一种新型的pH敏感高分子,其相转变pH（pHtr）在37℃下为6.0;当溶液pH〉6.0时,高分子溶解;pH〈6.0时,高分子很快从溶液中沉淀出来。在竞争型免疫测定中,偶联在高分子上的兔免疫球蛋白G（IgG）和标准兔IgG在溶液中竞争性地与有限量的异硫氰酸荧光素标记抗体反应,根据pHtr以下免疫复合物沉淀的特性进行分离,建立了均相免疫反应、异相分离的兔IgG新型测定方法,线性范围为100—1000μg／L;检出限为10μg/L。方法灵敏、快速且操作简便,由于pHtr较之以前合成的敏感高分子更接近于中性,分离时可降低对抗原-抗体免疫复合物造成的损坏。用于兔血清中免IgG的测量,结果令人满意。     

液体环境单分子免疫球蛋白G的原子力显微镜高分辨成像

原子力显微镜技术( AFM)具有纳米级高分辨成像能力,是研究生物大分子结构和功能的重要工具之一。制备合适的样品是获取高分辨成像的关键要素。本研究结合DNA折纸技术,将抗原分子修饰在DNA折纸上,通过分子识别作用,抗体分子与抗原分子特异性结合,形成由DNA折纸和抗原抗体复合物构成的纳米结构。利用DNA折纸在云母表面上的吸附特点,使得抗体分子选择性地吸附在衬底表面上,由此获得了液体环境中的单个地高辛抗体免疫球蛋白G( IgG)分子的“Y”超微结构形貌。本方法简单、方便,为AFM在单分子水平上检测和表征生物分子结构和功能提供帮助。     

蛋白A连续床亲和毛细管色谱柱的制备及性能考察

人免疫球蛋白 G(HIg G)是一种重要的生物大分子 ,是人血浆中的主要成分之一 ,通常采用免疫学的方法测定 .蛋白 A(Protein A)与免疫球蛋白 (HIg G)的 Fc区之间具有很强的特异性亲和作用 ,因而固载蛋白 A的亲和介质可用于免疫球蛋白及单克隆抗体的分离、纯化和分析测定[1～ 3 ] .根据固定相存在形式的不同 ,毛细管色谱柱主要有开管、填充和连续床柱 3种方式 .连续床具有相比高、易制备 (一步合成 )、孔径易控制、不需烧塞子和易改性等优点 .连续床与其它常用的亲和介质 (如球型凝胶颗粒、灌流色谱基质 [4、 5] 、膜介质 [6,7] 等 )相比具…     

小鼠血清IgG的蛋白G灌注亲和色谱行为的研究

通过实验考察了小鼠血清ＩｇＧ的蛋白Ｇ灌注亲和色谱行为,虽然未发现非特异性吸附,但在通常情况下对ＩｇＧ存在不可逆性吸附。洗脱液组成及ｐＨ的不同决定ＩｇＧ在灌注亲和色谱柱上具有不同的解离常数ＫＤ,产生不同的色谱行为。流动相的流速对ＩｇＧ与蛋白Ｇ的结合／解离动力学过程产生一定的影响。结果表明,对于小鼠血清中的ＩｇＧ灌注亲和色谱的分离,由于解离速率影响到传质过程,使之在高流速下的分离受到一定的限制。     

毛细管电泳法快速测定保健食品中免疫球蛋白G

建立了毛细管电泳法快速测定保健食品中免疫球蛋白G(IgG)含量的方法,成功测定了不同剂型(片剂、粉剂及胶囊)牛初乳保健品中IgG的含量。以37 cm×50μm(i.d.)未涂敷熔融石英毛细管为色谱分离柱,50 mmol/L四硼酸钾 65 g/L聚乙二醇20 000(1 mol/L氢氧化铯调pH 10.0)为运行缓冲液,于214 nm波长处检测。详细研究了影响实际样品中IgG分离及准确定量的关键因素,如添加剂的种类、浓度;运行及样品缓冲液的浓度及pH等。采用峰面积外标法定量。方法的精密度为2.1%(n=7);检出限为6.25 mg/L(S/N=3);线性范围为50~2000 mg/L;400 mg/L IgG迁移时间的相对标准偏差(RSD)为0.14%;峰面积的RSD为2.9%(n=7)。6 m in内即可实现保健食品中IgG的分离与测定,结果与产品标示值基本吻合。     

固载蛋白A交联聚甲基丙烯酸缩水甘油酯连续床亲合色谱柱的制备及性能考察

采用沉淀聚法“原位”（in-situ)聚合合成了交联聚甲基丙烯酸缩水甘油酯连续床色谱柱,对其进行化学改性后,分别得到含有11个碳原子间隔臂以及不含间隔臂键合了蛋白A的高效亲合色谱柱。考察了这两种色谱介质的性能,结果表明含有间隔臂的介质有一定的疏水性;对传统制备蛋白配基的亲合色谱介质的合成路线进行了改进;采用不含间隔臂的亲合柱测定了人血浆中人免疫球蛋白G（HIgG)的含量,所测得的定量标准曲线线性相关系数达到0．999;考察了流速对合成的连续床色谱柱柱压的影响,当流速高达9．0mL/min时,柱压也仅为6．5MPa;采用pH梯度对HIgG的不同亚基进行了分离。     

偶氮洋红G-SDS体系共振光散射法测定蛋白质

在十二烷基磺酸钠存在下及pH 1．98的Brittion-Robinson介质中,蛋白质与偶氮洋红G作用形成复合物,使最大波长421nm的共振光散射光谱得到加强,根据其共振光散射的增强程度,可定量测定蛋白质。十二烷基磺酸钠的加入,使灵敏度提高2．7倍。牛血清白蛋白、γ-球蛋白的线性范围分别为0.04～1．6、0．12～3．8mg／L,检出限分别为5．3、8．5μg/L。用于人血清、牛奶、豆浆、尿液中总蛋白质的测定,结果与经典的考马斯亮蓝法一致。     

顺序注射可更新表面固相荧光免疫法测定人血清中免疫球蛋白G

建立了采用芯片式微型流通池的测定人血清中免疫球蛋白G(IgG)的顺序注射可更新表面非均相荧光免疫分析法。将羊抗人IgG抗体固定于包被有蛋白A的Sephamse CL4B凝胶微珠,然后制备成固相抗体。用标记FITC的抗人IgG抗体作为第二抗体。固相抗体、血清试样和荧光标记第二抗体由顺序注射系统注入芯片式微型流通池,并在其中进行免疫反应生成夹心式抗体．抗原荧光复合物。荧光分光光度计通过光纤与流通池耦合测定截留于流通池中的抗体一抗原复合物荧光强度。一次测定完成后,微珠即被排出流通池。流通池经缓冲液清洗后即可进行下一次测定。体系经优化后,检出限为0．1mg／L IgG,分析速率达到11次／h。3．9mg／L IgG的日内和日间精密度(RSD)分别为1．7％和5．2％;校正曲线的线性范围为0．3—7．0mg／L IgG。所建立的方法已成功地应用于人血清中IgG的测定。     

Determination of Procaine Penicillin G and Penicillin G by Second Derivative Spectrophotometry in Pharmaceutical Products

Abstract

“Zero-crossing” derivative spectrophotometry has been used for determining binary mixtures of penicillin G and procaine penicillin G.

The procedure is rapid, simple, nondestructive, and does not require resolutions of equations.

Calibration graphs are linear between 2.0 and 50.0 μg mL^?1 of the penicillin G at 226.0 nm, and between 2.0 and 100.0 μg mL^?1 of procaine penicillin G at 319.0 nm, in the presence of each other. A complete and exhausive statistical analysis of the experimental data was realized to demonstrate the validity of method. The method was successfully applied to assay commercial injections of these drugs.     

Analysis of bovine immunoglobulin G in milk,colostrum and dietary supplements: a review

The immunoprotective properties of bovine milk immunoglobulin G (IgG) have led to a recent proliferation of nutritional products incorporating this protein. It has therefore become critical that reliable analytical techniques for the measurement of the IgG content in such products are available. This literature review surveys current methods of analysis for IgG, including separation-based or immuno-based concentration analysis. The review also discusses nutraceutical applications, regulatory issues, stability of IgG and the significance of primary reference material in IgG analysis.     

丽春红G 用于人血清样品中总蛋白的共振光散射测定

在酸性介质中 ,丽春红G (PonceauG ,PG)与牛血清白蛋白 (BSA)、人血清白蛋白 (HSA)、溶菌酶 (Lys)及γ 球蛋白 (γ IgG)等蛋白质作用产生共振光散射 (RLS)增强信号 ,最大散射峰位于 2 88nm处。在最佳酸度和离子强度下 ,增强RLS强度在 2 88nm处与蛋白质的浓度呈线性关系 ,用于测定BSA、HSA、Lys、γ IgG的检出限均在 2 5 μg L以下。本方法成功地应用于合成样和人血清样品的测定 ,测量结果与考马斯亮蓝法一致     

Immobilized enzymes in clinical and biochemical analysis : Applications to the Simultaneous Determination of Acetylcholine and Choline and to Determination of Lipids

Uses of immobilized enzyme mini-columns in flow-injection systems are described Simultaneous determination of ? × 10^?5 M choline and acetylcholine is achieved by using acetylcholinesterase and choline oxidase columns. A home-made amperometric detector is used to detec the hydrogen peroxide produced enzymatically. An ion-exchange column is used on-line to remove interferences at the amperometric detector during analysis of blood and brain samples. Immobilization of the lipid enzymes phospholipase-C and -D is described. These enzymes are used for the determination of phospholipids. Total phospholipids (1– mM) are determined with a combination of phospholipase-D, lipase and glycerol-3-phosphate oxidase. All the methods described are simple and reproducible and the immobilized enzymes show good stability.     

Binding of Glycans to the SARS CoV-2 Spike Protein,an Open Question: NMR Data on Binding Site Localization,Affinity, and Selectivity

We have used NMR experiments to explore the binding of selected glycans and glycomimetics to the SARS CoV-2 spike glycoprotein (S-protein) and to its receptor binding domain (RBD). STD NMR experiments confirm the binding of sialoglycans to the S-protein of the prototypic Wuhan strain virus and yield dissociation constants in the millimolar range. The absence of STD effects for sialoglycans in the presence of the Omicron/BA.1 S-protein reflects a loss of binding as a result of S-protein evolution. Likewise, no STD effects are observed for the deletion mutant Δ143–145 of the Wuhan S-protein, thus supporting localization of the binding site in the N-terminal domain (NTD). The glycomimetics Oseltamivir and Zanamivir bind weakly to the S-protein of both virus strains. Binding of blood group antigens to the Wuhan S-protein cannot be confirmed by STD NMR. Using ¹H,¹⁵N TROSY HSQC-based chemical shift perturbation (CSP) experiments, we excluded binding of any of the ligands studied to the RBD of the Wuhan S-protein. Our results put reported data on glycan binding into perspective and shed new light on the potential role of glycan-binding to the S-protein.     

LC–MS Determination and Pharmacokinetic Study of a Novel Sulfonylurea: Potential Hypoglycemic Agent in Rat Plasma

To support preclinical pharmacokinetic investigation of 1-[4-[2-(4-bromobenzene-sulfonaminoethyl)phenylsufonyl]-3-(trans-4-methylcyclohexyl)urea (G004), a rapid, sensitive and specific high-performance liquid chromatography–electrospray ionization mass spectrometry (LC–ESI-MS) method was developed and validated. Glibenclamide was employed as internal standard. After liquid–liquid extraction the analyte was analyzed on a Kromasil C₁₈ column (150 × 2.0 mm i.d.) with a mobile phase consisted of acetonitrile–water (0.05% acetic acid), 30:70 (v/v). The flow rate was 0.2 mL min⁻¹. Detection was performed on a quadrupole mass spectrometer using an electrospray ionization interface and the selected-ion monitoring (SIM) mode. The retention time was about 3.5 and 4.2 min for Glibenclamide and G004, respectively. The assay was linear over the concentration range of 2.0–500.0 ng mL⁻¹. Extraction Recovery of G004 in rat plasma was more than 87%. The intra- and inter-assay precision was lower than 11.5% (CV). This validated method was successfully applied to the pharmacokinetics of G004 in rats.     

Direct Spectrophotometric Determination of Calcium in Human Serum and Cerebrospinal Fluids with Amino G Acid Chlorophosphonazo

ABSTRACT

A novel spectrophotometric method based on amino G acid chlorophosphonazo (AGCPA) has been developed for measuring calcium in human serum and cerebrospinal fluids. The effects of experimental factors including pH, reagent concentrations, and interfering species on calcium determinations were investigated. In a neutral reaction media of pH 7.0, AGCPA reacts rapidly with calcium to form a stable and greenish blue complex, whose absorption maximum is at 670 nm. The molar absorptivity (?) of the complex is 7.2x10⁴ 1 mol^?1cm^?1, and the molar ratio of calcium to AGCPA in the complex is found to be 1:2. Beer's law is obeyed over the range 0.02-0.8 μg ml^?1 of calcium. No interferences were observed from the commonly coexisting species present in serum and cerebrospinal fluids. Compared to the reported and currently often used methods based on o-cresolphthalein complexone, arsenazo III and methylthymol blue, the proposed method in this work provides better analytical characteristics such as high sensitivity, good selectivity and neutral reaction media. In addition, the present method is simple and can be applied to the direct determination of calcium in human serum and cerebrospinal fluid samples with satisfactory results.